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SRX528865: GSM1376272: NBB2009-075; Homo sapiens; RNA-Seq
12 ABI_SOLID (AB 5500xl Genetic Analyzer) runs: 57.7M spots, 4.3G bases, 1.9Gb downloads

Submitted by: Gene Expression Omnibus (GEO)
Study: Alternative poly(A) in Alzheimer's disase
show Abstracthide Abstract
Alternative polyadenylation (APA) contributes to post-transcriptional regulation, but its role in Alzheimer's disease (AD) is largely unknown. Using high-resolution SQUARE multiple 3' primer-based sequencing, we discovered massive APA differences in temporal gyrus tissues from demented AD patients compared to either healthy controls or non-demented donors with AD neuropathology (NDWP). Advanced statistics, microfluidics RT-PCR and protein measurements validated known and novel APA-modified 3'-intact transcripts. Moreover, APA modifications, more than total transcript counts, distinguished AD patients from both controls and NDWP donors and identified cell type-characteristic, cognition-associated and neuropathology-related changes. AD-enhanced APA variants included known therapeutic targets of brain, vascular and autoimmune disorders, predicting co-involvement of these target genes in AD progression; AD/NDWP increases in 3'-intact proteinopathy-related hnRNP mRNAs were inversely associated with protein decreases, whereas NDWP-potentiated cognition was accompanied by distinct ATP and mitochondrial variants. APA variations thus provide a novel resource of unique value for both basic and translational neuroscience researchers. Overall design: Examination of poly adenylation sites in brain tissues of Alzheimer's disease patients, non-demented with Alzheimer's disease like pathology and non-demented without Alzheimer's disease like pathology.
Sample: NBB2009-075
SAMN02739919 • SRS599109 • All experiments • All runs
Organism: Homo sapiens
Library:
Instrument: AB 5500xl Genetic Analyzer
Strategy: RNA-Seq
Source: TRANSCRIPTOMIC
Selection: cDNA
Layout: SINGLE
Construction protocol: RNA was extracted with the SPLIT RNA extraction kit (Lexogen GmbH, Vienna, Austria) yielding the large RNA fraction with a lower cut-off size of 150 nt. Evaluation on an Bioanalyzer RNA Nano chip (Agilent Technologies) showed medium to high RNA quality (RIN of 6.2 – 8.3). Briefly, 4 µg Terminator-treated RNA was full-length reverse transcribed, and 1/20th of the purified cDNA was then amplified in one of 12 parallel PCR reactions. Each PCR reactions was set up with one universal 5’ primer and a 3’ primer selective for one of the 12 possible combinations of the two terminal nucleotides of the mRNA body, immediately upstream of the poly(A) tail. 200 ng of all 288 PCR products (24 RNA samples amplified separately in 12 matrix fields) were heat-fragmented and then ligated to SOLiD-compatible adapters. The libraries were PCR amplified in 17 cycles, with PCR primers indexing each sample with one out of 96 bar-codes. Three lane mixes were created, each from 96 libraries corresponding to 24 samples amplified in 4 matrix fields, dedicating equal molarities to each of the libraries. The three lane mixes SOR04 (selective 3’ primer nucleotides AC, AG, CA, GT), SOR05 (AA, AT, CC, CG) and SOR06 (CT, GA, GC, GG) were then further size-selected on a Pippin Prep automated gel elution system (Sage Biosciences, Beverly, MA, USA) in the range of 170 to 400 bp.
Experiment attributes:
GEO Accession: GSM1376272
Links:
External link:
Runs: 12 runs, 57.7M spots, 4.3G bases, 1.9Gb
Run# of Spots# of BasesSizePublished
SRR12653654,266,980320M130Mb2017-04-27
SRR12653664,296,950322.3M130Mb2017-04-27
SRR12653674,059,816304.5M125.4Mb2017-04-27
SRR12653686,494,534487.1M238.4Mb2017-04-27
SRR12653695,391,189404.3M190.3Mb2017-04-27
SRR12653706,373,058478M235Mb2017-04-27
SRR12653714,946,871371M142.3Mb2017-04-27
SRR12653725,542,746415.7M198.3Mb2017-04-27
SRR12653732,536,664190.2M82.2Mb2017-04-27
SRR12653744,070,328305.3M127.3Mb2017-04-27
SRR12653754,011,957300.9M135.7Mb2017-04-27
SRR12653765,748,228431.1M181Mb2017-04-27

ID:
729347

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